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直接测序、高分辨率熔解和变性高效液相色谱法检测突尼斯散发性结肠直肠癌患者的 KRAS 突变。

KRAS mutation detection in Tunisian sporadic coloractal cancer patients with direct sequencing, high resolution melting and denaturating high performance liquid chromatography.

机构信息

Laboratoire de Génétique, Immunologie et Pathologies Humaines, Faculté des Sciences de Tunis, Université de Tunis El Manar, Tunisia.

出版信息

Cancer Biomark. 2010;8(6):331-40. doi: 10.3233/CBM-2011-0222.

DOI:10.3233/CBM-2011-0222
PMID:22072121
Abstract

The Kirsten Rat Sarcoma (KRAS) oncogene has been introduced recently as a genetic biomarker for metastatic sporadic colorectal cancer prior to anti-EGFR treatment. Identifying patients with KRAS mutations that not respond to EGFR targeted therapies require sensitive, rapid and efficacious routine technique. We have attempted to evaluate the efficiency of three conventional methods: direct sequencing, HRM and DHPLC, to detect mutations in codon 12 and 13 of the KRAS exon2 gene. For this first Tunisian study on KRAS, we detected 45.83% of altered KRAS gene among 48 formalin-fixed paraffin-embedded sporadic colorectal adenocarcinoma patients. The use of HRM-sequencing allowed as enlarging the detected KRAS exon 2 mutations (22/48) in comparison with direct sequencing (17/48). DHPLC was used to confirm results when consensus was not observed between HRM and direct sequencing. This study brings an interesting data concerning an inter-method validation between sequencing and HRM in the investigation of sporadic colorectal cancer biomarker. It also shows that KRAS mutations occur at similar frequencies in Tunisian patients as in other populations; and suggests that the same genes are at play in sporadic CRC cancer, despite ethnic, geographical and environmental differences between countries.

摘要

Kirsten 鼠肉瘤(KRAS)癌基因最近被引入作为转移性散发性结直肠癌抗 EGFR 治疗前的遗传生物标志物。鉴定对 EGFR 靶向治疗无反应的 KRAS 突变患者需要敏感、快速和有效的常规技术。我们试图评估三种常规方法的效率:直接测序、高分辨率熔解(HRM)和变性高效液相色谱(DHPLC),以检测 KRAS 外显子 2 基因密码子 12 和 13 中的突变。对于这项关于 KRAS 的首例突尼斯研究,我们在 48 例福尔马林固定石蜡包埋的散发性结直肠腺癌患者中检测到 45.83%的 KRAS 基因改变。与直接测序(17/48)相比,HRM-测序法(22/48)可扩大检测到的 KRAS 外显子 2 突变。当 HRM 和直接测序之间没有达成共识时,DHPLC 用于确认结果。这项研究提供了有关在散发性结直肠癌生物标志物研究中测序和 HRM 之间的方法验证的有趣数据。它还表明,KRAS 突变在突尼斯患者中的发生频率与其他人群相似;并表明尽管国家之间存在种族、地理和环境差异,但相同的基因在散发性 CRC 癌症中起作用。

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